Promoter engineering enables overproduction of foreign proteins from a single copy expression cassette in Bacillus subtilis

生产过剩 枯草芽孢杆菌 绿色荧光蛋白 质粒 异源的 生物 发起人 分子生物学 表情盒 基因表达 细菌 生物化学 遗传学 基因 载体(分子生物学) 重组DNA
作者
Chaoyang Zhou,Bin Ye,Shan Cheng,Leizhen Zhao,Yuanxin Liu,Jiandong Jiang,Xin Yan
出处
期刊:Microbial Cell Factories [Springer Nature]
卷期号:18 (1) 被引量:58
标识
DOI:10.1186/s12934-019-1159-0
摘要

Bacillus subtilis is developed to be an attractive expression host to produce both secreted and cytoplasmic proteins owing to its prominent biological characteristics. Chromosomal integration is a stable expression strategy while the expression level is not ideal compared with plasmid expression. Thus, to meet the requirement of protein overexpression, promoter, as one of the key elements, is important. It is necessary to obtain an ideal promoter for overproduction of foreign proteins from a single copy expression cassette. The activity of promoter Pylb was further enhanced by optimizing the − 35, − 10 core region and upstream sequence (UP) by substituting both sequences with consensus sequences. The final engineered promoter exhibited almost 26-fold in β-galactosidase (BgaB) activity and 195-fold in super-folded green fluorescent protein (sfGFP) intensity than that of WT. The two proteins account for 43% and 30% of intracellular proteins, respectively. The promoter was eventually tested by successful extracellular overproduction of Methyl Parathion Hydrolase (MPH) and Chlorothalonil hydrolytic dehalogenase (Chd) to a level of 0.3 g/L (144 U/mL) and 0.27 g/L (4.4 U/mL) on shake-flask culture condition. A strong promoter was engineered for efficient chromosomally integrated expression of heterologous proteins.
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